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Detection of Cell Surface Ligands for Human Synovial γδ T Cells

Lack of understanding of the nature and physiological regulation of γδ T cell ligands has considerably hampered full understanding of the function of these cells. We developed an unbiased approach to identify human γδ T cells ligands by the production of a soluble TCR-γδ (sTCR-γδ) tetramer from a sy...

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Autores principales: Collins, Cheryl, Lui, Yuan, Santos, Ana Mafalda, Ballif, Bryan A., Gogerly-Moragoda, Anisha Mahalya, Brouwer, Heather, Ross, Robin, Balagurunathan, Kuberan, Sharma, Sumana, Wright, Gavin J., Davis, Simon, Budd, Ralph C.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: AAI 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6804759/
https://www.ncbi.nlm.nih.gov/pubmed/31548331
http://dx.doi.org/10.4049/jimmunol.1900451
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author Collins, Cheryl
Lui, Yuan
Santos, Ana Mafalda
Ballif, Bryan A.
Gogerly-Moragoda, Anisha Mahalya
Brouwer, Heather
Ross, Robin
Balagurunathan, Kuberan
Sharma, Sumana
Wright, Gavin J.
Davis, Simon
Budd, Ralph C.
author_facet Collins, Cheryl
Lui, Yuan
Santos, Ana Mafalda
Ballif, Bryan A.
Gogerly-Moragoda, Anisha Mahalya
Brouwer, Heather
Ross, Robin
Balagurunathan, Kuberan
Sharma, Sumana
Wright, Gavin J.
Davis, Simon
Budd, Ralph C.
author_sort Collins, Cheryl
collection PubMed
description Lack of understanding of the nature and physiological regulation of γδ T cell ligands has considerably hampered full understanding of the function of these cells. We developed an unbiased approach to identify human γδ T cells ligands by the production of a soluble TCR-γδ (sTCR-γδ) tetramer from a synovial Vδ1 γδ T cell clone from a Lyme arthritis patient. The sTCR-γδ was used in flow cytometry to initially define the spectrum of ligand expression by both human tumor cell lines and certain human primary cells. Analysis of diverse tumor cell lines revealed high ligand expression on several of epithelial or fibroblast origin, whereas those of hematopoietic origin were largely devoid of ligand. This allowed a bioinformatics-based identification of candidate ligands using RNAseq data from each tumor line. We further observed that whereas fresh monocytes and T cells expressed low to negligible levels of TCR-γδ ligands, activation of these cells resulted in upregulation of surface ligand expression. Ligand upregulation on monocytes was partly dependent upon IL-1β. The sTCR-γδ tetramer was then used to bind candidate ligands from lysates of activated monocytes and analyzed by mass spectrometry. Surface TCR-γδ ligand was eliminated by treatment with trypsin or removal of glycosaminoglycans, and also suppressed by inhibition of endoplasmic reticulum–Golgi transport. Of particular interest was that inhibition of glycolysis also blocked TCR-γδ ligand expression. These findings demonstrate the spectrum of ligand(s) expression for human synovial Vδ1 γδ T cells as well as the physiology that regulates their expression.
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spelling pubmed-68047592019-10-25 Detection of Cell Surface Ligands for Human Synovial γδ T Cells Collins, Cheryl Lui, Yuan Santos, Ana Mafalda Ballif, Bryan A. Gogerly-Moragoda, Anisha Mahalya Brouwer, Heather Ross, Robin Balagurunathan, Kuberan Sharma, Sumana Wright, Gavin J. Davis, Simon Budd, Ralph C. J Immunol Clinical and Human Immunology Lack of understanding of the nature and physiological regulation of γδ T cell ligands has considerably hampered full understanding of the function of these cells. We developed an unbiased approach to identify human γδ T cells ligands by the production of a soluble TCR-γδ (sTCR-γδ) tetramer from a synovial Vδ1 γδ T cell clone from a Lyme arthritis patient. The sTCR-γδ was used in flow cytometry to initially define the spectrum of ligand expression by both human tumor cell lines and certain human primary cells. Analysis of diverse tumor cell lines revealed high ligand expression on several of epithelial or fibroblast origin, whereas those of hematopoietic origin were largely devoid of ligand. This allowed a bioinformatics-based identification of candidate ligands using RNAseq data from each tumor line. We further observed that whereas fresh monocytes and T cells expressed low to negligible levels of TCR-γδ ligands, activation of these cells resulted in upregulation of surface ligand expression. Ligand upregulation on monocytes was partly dependent upon IL-1β. The sTCR-γδ tetramer was then used to bind candidate ligands from lysates of activated monocytes and analyzed by mass spectrometry. Surface TCR-γδ ligand was eliminated by treatment with trypsin or removal of glycosaminoglycans, and also suppressed by inhibition of endoplasmic reticulum–Golgi transport. Of particular interest was that inhibition of glycolysis also blocked TCR-γδ ligand expression. These findings demonstrate the spectrum of ligand(s) expression for human synovial Vδ1 γδ T cells as well as the physiology that regulates their expression. AAI 2019-11-01 2019-09-23 /pmc/articles/PMC6804759/ /pubmed/31548331 http://dx.doi.org/10.4049/jimmunol.1900451 Text en Copyright © 2019 The Authors https://creativecommons.org/licenses/by/4.0/ This article is distributed under the terms of the CC BY 4.0 Unported license.
spellingShingle Clinical and Human Immunology
Collins, Cheryl
Lui, Yuan
Santos, Ana Mafalda
Ballif, Bryan A.
Gogerly-Moragoda, Anisha Mahalya
Brouwer, Heather
Ross, Robin
Balagurunathan, Kuberan
Sharma, Sumana
Wright, Gavin J.
Davis, Simon
Budd, Ralph C.
Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title_full Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title_fullStr Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title_full_unstemmed Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title_short Detection of Cell Surface Ligands for Human Synovial γδ T Cells
title_sort detection of cell surface ligands for human synovial γδ t cells
topic Clinical and Human Immunology
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6804759/
https://www.ncbi.nlm.nih.gov/pubmed/31548331
http://dx.doi.org/10.4049/jimmunol.1900451
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